摘要
该文通过改进双向电泳方法克服了膜蛋白由于有疏水性而很难进入双向电泳第一相——等电聚焦电泳凝胶,以及由于从蔗糖密度梯度离心中分离得到的液泡前体富含干扰等电聚焦电泳效果的蔗糖等两大难点,成功地分离了通过蔗糖密度梯度离心分离得到的液泡前体蛋白,并使膜蛋白进入了双向电泳凝胶.双向电泳后分离到约200余个蛋白质点,用基质辅助激光解吸/电离飞行时间串联质谱(MS/MS)进行肽质量指纹谱分析,并通过数据库检索进行蛋白质鉴定与功能预测,分析的23个蛋白中有13个在数据库中没有找到相对应的吻合蛋白,查询到的10个吻合蛋白中有6个功能未知.
It is difficult for membrane proteins to get into 2-D gel because of their hydrophobic properties and the contaminations of carbohydrates in protein samples also affect the results of 2-D gel. The modified 2-D electrophoresis technique described in this paper overcomes these two difficulties, and have successfully separated proteins from sucrose gradient ultracentrifugation and got membrane proteins into 2-D gel. Pro teomic analysis was then performed on proteins from prevacuolar compartment. Around 200 protein spots were separated on the 2-D gel,23 protein spots were cut out form the gel and subjected to MS/MS analysis. After database searching, 13 proteins did not hit matching proteins, with the 10 proteins that hit matching proteins, 4 of them have known protein function, 6 of which turned out to be unknown or unnamed proteins.
出处
《华东师范大学学报(自然科学版)》
CAS
CSCD
北大核心
2005年第2期91-97,共7页
Journal of East China Normal University(Natural Science)
基金
香港自然科学基金资助项目(CUHK4260)
关键词
双向电泳
肽质量指纹谱
液泡前体
膜蛋白
烟草
2-D electrophoresis
peptide mass finger print
prevacuolar compartment
membrane protein
tobacco